Gibbons Don L, Ahn Anna, Liao Maofu, Hammar Lena, Cheng R Holland, Kielian Margaret
Department of Cell Biology, Albert Einstein College of Medicine, Bronx, New York 10461, USA.
J Virol. 2004 Apr;78(7):3312-8. doi: 10.1128/jvi.78.7.3312-3318.2004.
A prevailing model for virus membrane fusion proteins has been that the hydrophobic fusion peptide is hidden in the prefusion conformation, becomes exposed once the fusion reaction is triggered, and then either inserts into target membranes or is rapidly inactivated. This model is in general agreement with the structure and mechanism of class I fusion proteins, such as the influenza virus hemagglutinin. We here describe studies of the class II fusion protein E1 from the alphavirus Semliki Forest virus (SFV). SFV fusion is triggered by low pH, which releases E1 from its heterodimeric interaction with the E2 protein and induces the formation of a stable E1 homotrimer. The exposure and target membrane interaction of the E1 fusion peptide (residues 83 to 100) were followed using a monoclonal antibody (MAb E1f) mapping to E1 residues 85 to 95. In agreement with the known structure of SFV and other alphaviruses, the fusion peptide was shielded in native SFV particles and exposed when E1-E2 dimer dissociation was triggered by acidic pH. In contrast, the fusion peptide on purified E1 ectodomains (E1()) was fully accessible at neutral pH. Functional assays showed that MAb E1f binding at neutral pH prevented subsequent low-pH-triggered E1() interaction with target membranes and trimerization. E1(*) was not inactivated by low pH when treated either in the absence of target membranes or in the presence of fusion-inactive cholesterol-deficient liposomes. Thus, the membrane insertion of the E1 fusion peptide is regulated by additional low-pH-dependent steps after exposure, perhaps involving an E1-cholesterol interaction.
关于病毒膜融合蛋白的一个普遍模型是,疏水融合肽在融合前构象中是隐藏的,一旦融合反应被触发就会暴露出来,然后要么插入靶膜,要么迅速失活。该模型与I类融合蛋白(如流感病毒血凝素)的结构和机制总体上一致。我们在此描述了对甲病毒塞姆利基森林病毒(SFV)的II类融合蛋白E1的研究。SFV融合由低pH触发,这使其E1从与E2蛋白的异二聚体相互作用中释放出来,并诱导形成稳定的E1同源三聚体。使用靶向E1第85至95位残基的单克隆抗体(MAb E1f)追踪E1融合肽(第83至100位残基)的暴露和与靶膜的相互作用。与SFV和其他甲病毒的已知结构一致,融合肽在天然SFV颗粒中被屏蔽,当酸性pH触发E1-E2二聚体解离时暴露出来。相比之下,纯化的E1胞外域(E1())上的融合肽在中性pH下是完全可及的。功能测定表明,中性pH下MAb E1f的结合阻止了随后低pH触发的E1()与靶膜的相互作用和三聚化。当在没有靶膜的情况下或在存在融合无活性的胆固醇缺陷脂质体的情况下处理时,E1(*)不会被低pH失活。因此,E1融合肽的膜插入在暴露后由额外的低pH依赖性步骤调节,可能涉及E1-胆固醇相互作用。